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重组L-蛋氨酸γ-裂解酶(一种抗癌剂)的高水平表达与大量结晶

High-level expression and bulk crystallization of recombinant L-methionine gamma-lyase, an anticancer agent.

作者信息

Takakura Tomoaki, Ito Takaomi, Yagi Shigeo, Notsu Yoshihide, Itakura Takashi, Nakamura Takumi, Inagaki Kenji, Esaki Nobuyoshi, Hoffman Robert M, Takimoto Akio

机构信息

Discovery Research Laboratories, Shionogi & Co., Ltd., Amagasaki, Hyogo, Japan.

出版信息

Appl Microbiol Biotechnol. 2006 Mar;70(2):183-92. doi: 10.1007/s00253-005-0038-2. Epub 2005 Jul 13.

DOI:10.1007/s00253-005-0038-2
PMID:16012835
Abstract

L-Methionine gamma-lyase is a pyridoxal 5'-phosphate-dependent enzyme which has tumor selective anticancer activity. An efficient production process for the recombinant enzyme was constructed by using the overexpression plasmid in Escherichia coli, large-scale cultivation, and practical crystallization on an industrial scale. The plasmid was optimized with a promoter and the region of the ribosome-binding site. Plasmid pMGLTrc03, which has a trc promoter and a spacing of 12 nucleotides between the Shine-Dalgarno sequence and the ATG translation initiation codon, was selected as the most suitable plasmid. The transformants produced the enzyme, which intracellularly accumulated at 2.1 mg/ml as an active form and accounted for 43% of the total proteins in the soluble fraction by simple batch fermentation using a 500-l fermentor. The crystals were directly obtained from crude enzyme with 87% yield by a crystallization in the presence of 9.0% polyethylene glycol 6000, 3.6% ammonium sulfate, and 0.18 M sodium chloride using a 100-l crystallizer. After recrystallization, the enzyme was purified by anion-exchange column chromatography to remove endotoxins and by gel filtration for polishing. We prepared 600 g of purified enzyme with a low endotoxin content of sufficient quality for therapeutical use, with a 41% overall yield in the purification process.

摘要

L-蛋氨酸γ-裂解酶是一种依赖于磷酸吡哆醛5'-磷酸的酶,具有肿瘤选择性抗癌活性。通过在大肠杆菌中使用过表达质粒、大规模培养以及工业规模的实际结晶,构建了一种重组酶的高效生产工艺。该质粒通过启动子和核糖体结合位点区域进行了优化。具有trc启动子且Shine-Dalgarno序列与ATG翻译起始密码子之间间隔12个核苷酸的质粒pMGLTrc03被选为最合适的质粒。通过使用500升发酵罐进行简单分批发酵,转化体产生了该酶,其以活性形式在细胞内积累至2.1毫克/毫升,占可溶性部分总蛋白的43%。通过在含有9.0%聚乙二醇6000、3.6%硫酸铵和0.18 M氯化钠的条件下使用100升结晶器进行结晶,直接从粗酶中以87%的产率获得晶体。重结晶后,通过阴离子交换柱色谱法去除内毒素,并通过凝胶过滤进行精制来纯化该酶。我们制备了600克内毒素含量低且质量足以用于治疗的纯化酶,纯化过程的总产率为41%。

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